Method and composition for increasing branching and flowering response in plants

ABSTRACT

A unique fusion gene is disclosed which is useful for transforming a wide range of plants, resulting in a significant alteration of the plant phenotype with respect to shoot and floral tissue response, but not affecting root growth or function. The gene construct includes an ACC oxidase promoter to drive an ipt coding sequence that expresses IPT at certain stages of plant maturation and in certain tissues of the shoot. Exemplary transformations include chrysanthemum and tobacco, both of which exhibit increased branching in the vegetative shoot and increased bud count in the generative shoot.

RELATED APPLICATIONS

The instant application claims the benefit of U.S. Provisional Application No. 60/680,403, filed May 12, 2005. The entire contents of the aforementioned application are hereby incorporated herein by reference.

BACKGROUND

Transgenic or recombinant plants are of increasing interest because of the potential to control phenotypic traits as well as to produce large quantities of commercially useful products. Plants have been employed to overproduce heterologous proteins and in principle can produce a wide range of products, including high value proteins and certain pharmaceuticals. Transgenic plants with visually attractive phenotypes are particularly desirable as a source of economic benefit to horticulturists and to florist retailers, while transgenic agronomic crops with enhanced production traits are of economic benefit to food producers and consumers.

Genetically modified plants for agricultural products are already on the market, including herbicide, insect and virus resistant crop plants. Some of the better-known crops engineered for herbicide resistance include soybeans, maize, rapeseed, sugar beet, rice and cotton. Maize, potatoes, tomatoes and cotton have been modified for insect resistance.

Food source plants can be engineered to improve traits that affect nutritional value; for example, elevated iron in rice and wheat, higher amino acid content in potatoes, seedless fruits and increased carotenoids in rice and tomatoes. Recent efforts have turned to produce recombinant plants with maximal desired plant product at a selected harvest time (patent publication 20030093836, May 15, 2003) or to significantly increase a desired expressed product by targeting protein product accumulation in a targeted tissue (patent publication 20040117874, Jun. 17, 2004). Of particular interest are plants engineered to increase oil production; for example, canola oil, which is considered more healthful than trans fats and oils.

Cytokinins play a role in many growth and developmental processes in plants, such as apical dominance, cell differentiation, flowering, fruit set and ripening, leaf senescence and seed germination. The effects of cytokinins on plants can be exploited for agricultural and horticultural purposes through either exogenous application of cytokinin or endogenous manipulation of cytokinin metabolism. In Hatiora gaetneri for example, flower bud number can be more than doubled in response to a spray application of synthetic cytokinins (Boyle, 1995). The efficacy of exogenous spray applications is limited however, because flowers and leaves do not readily absorb cytokinins and movement of cytokinins within the plant is limited.

Alternatively, it has been reported that endogenous levels of cytokinins can be modified by integrating the ipt gene into the plant genome. The ipt gene encodes the enzyme isopentenyl transferase, which catalyzes the rate-limiting step in cytokinin biosynthesis. A number of promoters, including those inducible by heat, wounding, or light, have been used to drive ipt gene expression. Unfortunately, most of the resulting ipt transgenic plants exhibit morphological abnormalities since overproduction of cytokinins interferes with so many developmental processes (Gan and Amasino, 1997).

Transgenic plants that overproduce cytokinins tend to show reduced stature, release of apical dominance, changes in vascular development, and in some cases, inhibited root growth (Ainley, et al., 1993) In one study, Li, et al. (1992) fused the ipt gene to the auxin-inducible SAUR promoter. This promoter is primarily active in elongating tissue and SAUR-ipt plants expressed elevated levels of cytokinins in these tissues. SAUR-ipt plants displayed reduced stature, increased axillary bud development, reduced root initiation and growth, and exhibited complex and variable changes in senescence.

DEFICIENCIES IN THE ART

Commercially attractive plants are an economic asset for florists and businesses related to horticulture. Plants that produce abundant foliage and flowers without use of expensive external application of chemical agents would have economic benefits by decreasing labor and materials costs. Currently, some phenotypic traits such as cytokinin-controlled bud and leaf development are managed by application of relatively expensive chemicals, adding significantly to the cost of large growers' operations. There is a need for producing desirable plant phenotypes without excessive labor costs and in a controlled manner.

In ornamental horticulture, a significant proportion of all chemical growth regulators applied by growers are used to enhance plant form and aesthetic appearance; e.g., 78% of the 41,305 pounds (active ingredient) of chemical regulators were applied to greenhouse and nursery crops in the U.S. in 1993 were used to enhance aesthetic appearance. This adds not only to expense but also to environmental concerns of exposure to chemicals with possible hormonal effects. There is a need to develop plants that develop the desired phenotypes without need to apply external agents.

Most phenotypic characteristics in plants are developed by controlled crosses, which may or may not result in commercially desirable traits. Such crosses when successful in producing a desirable phenotype may result in sterile hybrids and incur high costs because of time and manpower required for development. Thus transgenic plants exhibiting desirable phenotypes and which can be readily propagated true to type would be desirable for commercial and economic reasons.

SUMMARY OF THE INVENTION

The present invention provides methods that address several deficiencies in certain types of commercial horticultural crops by providing transgenic plants with highly desirable phenotypes. The methods take advantage of the normal endogenous controls for development in the wild-type plant. It has been shown that a plant transformed with the described expression vector is capable of altering the normal ratio of auxin to cytokinin in the plant when endogenous stimuli are generated in the plant. Expression of the transgene results in predictable phenomic response, typically observed as increased branching in the vegetative shoot and increased bud count in the generative shoot compared with the non-transgenic plant.

Cytokinins play important roles in regulating plant growth and development. In developing the present invention, the gene coding for isopentenyl transferase (ipt) was placed under the control of a 0.918 kb fragment, including the 97 bp of 5′ UTR leader sequence plus the 821 bp of the untranscribed sequence, of the ACC oxidase gene promoter from Lycopersicon esculentum (LEACO1) and introduced into Nicotiana tabacum (cv. Havana), Dendranthema×grandiflorum (cv. Iridon), Euphorbia pulcherrima (cvs Red Success and Winter Rose Dark Red), and Creeping Bentgrass (Agrostis palustris).

T₁ generation LEACO1_(0.821 kb)-ipt tobacco lines displayed a range of growth habits from plants that appeared similar to the wild type in overall stature and branching habit but produced a greater number of flower buds (lines N2 and N8) to plant lines that expressed shoot characteristics typical of constitutive cytokinin expression (lines N1 and N4). For plants at one end of the phenology spectrum, transgenic tobacco plants displayed a dramatic increase in the number of flower buds compared to non-transgenic plants. This phenotype was often observed on plants with an otherwise normal growth habit. The phenotypes associated with LEACO1_(0.821 kb)-ipt transgenic chrysanthemum plants were even more varied; e.g., in one study, non-transgenic chrysanthemums averaged 2.67 laterals per plant following a mechanical pinch. In comparison, the average number of laterals per plant in 29 individual LEACO1_(0.821 kb)-ipt lines covered a continuous range from 2.17 to 9.17 laterals per plant. The average number of flower buds per plant for the 29 transgenic lines ranged from 16.8 to 154.7 compared to 15.5 for the non-transgenic wild-type plant as shown by the data provided herein. This range allows transgenic lines to be selected to meet any aesthetic or production goal, from a modest increase in flower bud and branch number to a dramatic increase in flower bud and branch number.

Plants at one end of the phenology spectrum were characterized by increased lateral branch development, shorter internodes, and fewer buds on the main stem. Isolated leaves of transgenic tobacco plants showed a significantly prolonged retention of chlorophyll under dark incubation (25° C. for 20 days). Leaves of non-transformed plants senesced gradually under the same conditions.

Analysis of ipt expression indicated a marked increase in gene expression in transgenic tobacco. Experiments with LEACO1_(0.821 kb)-gus transgenic tobacco plants suggested auxin and ethylene involvement in induction of LEACO1_(0.821 kb) promoter activity. The LEACO1_(0.821 kb)-ipt fusion gene has potential utility for improving certain ornamental and agricultural crop species by increasing flower bud initiation and altering branching habit.

Many crops are expected to benefit from the effects observed with transformations using gene constructs such as the ipt chimera disclosed. Almost all ornamental plants are considered more aesthetically pleasing when they display a compact, well-branched phenotype with lots of flowers. Field grown grain crops are also expected to be enhanced because an increase in the number of flowers, fruits or seeds produced per plant represents increased productivity.

The present invention provides an isolated polynucleotide comprising a nucleic acid that encodes an isopentenyltransferase (IPT) and a nucleic acid encoding a heterologous promoter. The encoding nucleic acid is a fusion of the IPT gene and the promoter gene, preferably in a construct where both genes are in an open reading frame such that when IPT polypeptide is expressed in a plant, stimulation of one or more plant cytokinins occurs.

The IPT gene, ipt, employed will be an entire gene, such as a bacterial gene, preferably from Agrobacterium tumefaciens. Of course due to the degeneracy of the genetic code, there are numerous replacement codons that will provide a particular amino acid and thus many substitutions can be made in a coding region without changing the primary structure of the encoded polypeptide. Additionally, it is contemplated that one may “plantize” ipt codons; i.e., substitute preferred amino acid codons in order to optimize expression for a particular plant species. Certain other substitutions in the coding region may also be made, such as those that substitute like amino acids; e.g., replacing one neutral amino acid codon with another neutral amino acid codon.

Likewise, mutant ipt or truncated ipt genes are also useful, so long as the chimeric fusion with a heterologous promoter gene is capable of being transferred into a plant cell and the encoded IPT expressed in the plant.

The ipt gene need not have a sequence identical to the bacterial ipt employed to illustrate the invention. So long as substantially similar activity is present and the construct is capable of stimulating endogenous cytokinin production in a transformed plant, the ipt nucleic acid sequence can be 80%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 97%, or 99% identical to the exemplary ipt.

An important aspect of the invention is the heterologous promoter employed to construct the fusion gene. For illustration, the LEACO_(0.821 kb) promoter fragment from the LEACO1 gene was fused to ipt gene. This gene is found in tomato plants, but homologs can be found in other plants, including melon, pea, and petunia. The leaco-1 gene codes for the amino cyclopropane carboxylic acid (ACC) oxidase (ACO) system and acts to convert ACC into ethylene. The several ACO genes cloned from a number of plant species are known and include leaco-1, leaco-2, leaco-3 from tomato, ps-ACO-1 from pea, ACO1, 3 and 4 from petunia and several from melon. In the present invention, the promoter from Leaco-1 gene (SEQ ID NO: 9) can readily be replaced with similar promoters from the above mentioned leaco genes in other plants, or by heterologous promoters with identities of 75, 76, 77, 78, 79, 80, 81, 82, 83, 84, 85, 86, 87, 88, 89, 90, 91, 92, 93, 94, 95, 96, 97, 98, or 99% so long as expression of the chimera in a selected plant is capable of stimulating cytokinin production.

The invention also comprises expression vectors harboring the chimeric genes constructed from an IPT-encoding nucleic acid, e.g. SEQ ID NO:5, and a heterologous promoter such as an ACO promoter. Particular examples of promoters are those encoded by the nucleic acid sequences of SEQ ID NO: 6 and SEQ ID NO:7. The ipt gene would be expected to have similar effect at identities of at least 80-90% of SEQ ID NO:5.

In other aspects of the invention, a host plant cell comprising the described expression vectors is contemplated, including transgenic plants propagated from such plant cells. Plants from which cells may be obtained or used for transformations include tobacco, chrysanthemum, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, watermelon and bent-grass; as well as the related species that are included in the respective plant families.

In particular embodiments, the invention also includes an isolated nucleic acid sequence comprising the nucleic acid sequence selected from the group consisting of SEQ ID NO: 6-7 in open reading frame with a nucleic acid encoding a heterologous isopentenyl transferase (IPT).

Another embodiment is an isolated nucleic acid sequence encoding isopentenyl transferase (IPT) fused 5′ with an ACO promoter capable of expressing the IPT in a plant. More particularly, the nucleic acid sequence is SEQ ID NO:5 fused with a nucleic acid having the sequence of SEQ ID NO: 6 (LEACO1_(0.821 kb) promoter plus the 97 bp UTR leader sequence) or SEQ ID NO:7.

Transgenic plants transformed with the disclosed LEACO1_(0.821 kb)-ipt constructs are a particularly important aspect of the invention. These transformed plants exhibit significantly increased branching and flower bud numbers compared to the untransformed plants of the same species. Particularly significant results have been demonstrated with chrysanthemum and flowering tobacco and are expected to be similar in several horticulturally important plants, including poinsettia, tomato and creeping bent-grass and in agriculture plants that are used for canola oil production. Other plants include tobacco, chrysanthemum, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, and watermelon, as well as related species. Exemplary families include the Cruciferae, Cucubitaceae, Compositae, Solanaceae, Euphorbiaceae, Gramineae, Leguminosae, and Rosaceae. In the Rosaceae there are over 3200 species with many important horticultural species such as plums, peaches, cherries, apricots and almonds in the genus Prunus. In the Compositae, there are over 20,000 species including many of the most popular ornamental species such as chyrsanthemum, asters, sunflower, marigold and the like. The Gramineae family includes many of the world's most important grain crops including rice, wheat, oats, barley, rye, and maize. It also includes sugar cane, important structural species such as bamboo, forages used for animal feeds and many important ornamental and turf species.

The invention also includes progeny of the described transgenic plants and seeds from these plants. The progeny show the same enhanced phenotypic traits as the parent. DNA analysis shows that one or more copies of the transgene can be incorporated into plant genome. Depending on the position of incorporation, the phenotypes; e.g., increased bud number and leaf branching, may vary in different plants transformed with the same expression vector; however, it is believed that vegetative propagation of a plant with highly desirable phenotype will result in substantially identical clones, allowing elimination of plants that do not have marketable appearance or productivity.

Related aspects of the invention include methods for increasing endogenous cytokinin levels in a plant, comprising transforming a plant with a transgene comprising an isopentenyltransferase (IPT)-encoding nucleic acid fused with an aminocyclopropane carboxylic acid oxidase promoter (ACO)-encoding nucleic acid. Expression of the transgene in the plant causes increased cytokinin levels in the transformed compared with a non-transformed plant of the same species. The increased cytokinin levels modify selected phenotypic traits in the maturing transgenic plant and particularly affect readily detectable changes such as time of senescence, increased lateral branch development and increased flower bud development (e.g. more buds initiated) when compared with untransformed plants of the same species. Particularly suitable plants for transformation include tobacco, chrysanthemum, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, watermelon and bent-grass, as well as related species.

Preferred ACO promoters for use in constructing the described chimeric genes include leaco1, leaco2 and leaco3, such as promoters having the nucleic acid sequence of SEQ ID NO. 6, SEQ ID NO:7 or SEQ ID NO: 12.

The methods described for the transgenic plants of the invention will have increased levels of cytokinins where endogenous production of these cytokinins can be affected by expression of the isopentenyltransferase gene under control of an ACC oxidase gene promoter fragment. Accordingly, expression of the IPT gene will be responsive to increased levels of the auxin indoleacetic acid or ethylene pathway activity in a transformed plant.

Overall and in general therefore, the invention includes expression vectors comprising any of the described fusion polypolypeptides encoded by a chimeric gene constructed from an ipt gene and an ACO promoter sequence. Also included are host plant cells and transgenic plants harboring the disclosed expression vectors.

For commercial purposes, and of use to growers who may wish to further develop plants in the manner disclosed, a packaged kit is contemplated. Such a kit may include a LEACO1_(0.821 kb)-ipt chimera comprised within a suitable transfection plasmid and directions for use of the plasmid suitable for various plant species.

BRIEF DESCRIPTION OF THE FIGURES

FIG. 1. Chimeric ACO-IPT construct in pBin binary vector

FIG. 2. Biosynthetic pathway for ethylene biosynthesis.

FIG. 3. Schematic diagram of typical phenotype for species with strong apical dominance shows elongation of lateral buds after removal (pinching) of apical buds in comparison with a LEACO1_(0.821 kb)-ipt transgenic line from the same species. The LEACO1_(0.821 kb)-ipt line exhibits increased lateral branch and bud development in the absence of apical bud removal.

FIG. 4. PCR analysis of putative transgenic LEACO1_(0.821 kb)-ipt tobacco plants and Southern blot analysis of genomic DNA isolated from tobacco plants. As expected, transgenic plants carried the 0.918 kb fragment comprised of the 0.821 kb LEACO1 promoter plus the 97 bp UTR leader sequence (A) and also showed a 0.52 kb fragment of the ipt gene (B). Lane 1: 1-kb ladder; Lane 2: Positive control (plasmid LEACO1_(0.821 kb)-ipt-nos); Lane 3: Negative control (wild type tobacco); Lanes 4-8: Putative transgenic tobacco lines. Southern blot analysis (C) of genomic DNA isolated from the wild type tobacco and LEACO1_(0.821 kb)-ipt transgenic tobacco lines (T₁ generation) representing both of the distinct phenotypic groups. The DIG-labeled 0.52 kb fragment of the ipt gene from LEACO1_(0.821 kb)-ipt-nos plasmid DNA was used as a probe. Two copies of the ipt gene were detected in some lines (such as N1 and N4, in lanes 2 and 3 respectively) while a single copy of the gene was detected in other lines that produced a distinct phenotypic characteristic (lines N2 and N8 in lanes 4 and 5 respectively). Non-transformed wild type Nicotiana tabacum DNA (Lane 1) served as a negative control and the ipt fragment was not detected. Plasmid DNA was used as a positive control (Lane 6).

FIG. 5. Number of flower buds in wild-type (FIG. 5A) and transformed by the LEACO1_(0.821 kb) construct (FIG. 5B) in tobacco plants.

FIG. 6. Phenomic responses observed in tobacco plants containing the ipt gene under control of the LEACO1_(0.821 kb) promoter varied widely. Plant N1 (FIG. 6A) displayed normal growth habit with increased flower bud number when compared with wild-type plants. Plant N4 (FIG. 6B) is the more extreme phenotype observed when transgenic lines contained multiple copies of the transgene or overexpressed the ipt gene. In chrysanthemum, phenotype of LEACO1_(0.821 kb)-ipt plants also varied widely but, unlike tobacco, many very highly desirable plant forms were observed.

FIG. 7. Ethephon suppressed ipt expression in LEACO1_(0.821 kb)-ipt tobacco lines. RT-PCR analysis was used to detect changes in ipt expression in transgenic lines after treatment with the ethylene-generating compound ethephon. Lane 1: LEACO1_(0.821 kb)-ipt (line N2) without ethephon treatment; Lane 2: LEACO1_(0.821 kb)-ipt (line N2) 24 h after ethephon treatment; Lane 3: LEACO1_(0.821 kb)-ipt (line N4) without ethephon treatment; Lane 4: LEACO1_(0.821 kb)-ipt (line N4) 24 h after ethephon treatment; Lane 5: wild type tobacco without ethephon treatment; Lane 6: wild type tobacco 24 h after ethephon treatment.

FIG. 8. Excised leaves of LEACO1_(0.821 kb)-ipt tobacco lines showed delayed senescence under prolonged dark conditions. Leaves from wild type tobacco (cv. Havana) and LEACO1_(0.821 kb)-ipt transgenic lines were detached, plated onto wet filter paper, and stored in the dark at 25° C. The chlorophyll content (□g/g FW) was measured immediately after leaves were detached and then periodically over a 40-day period. Chlorophyll in wild type leaves declined rapidly during the first 10-day period, but in leaves from LEACO1_(0.821 kb)-ipt plants, 50% of the initial chlorophyll concentration remained after 20 days in the dark. Leaves from the LEACO1_(0.821 kb)-ipt line that showed the highest ipt expression levels (N4) retained 30% of initial chlorophyll levels for up to 40 days. Means at each sample date labeled with the same letters are not significantly different according to Tukey's multiple comparison test with a family error rate of 0.05.

FIG. 9. Branching and flower bud count differed markedly for wild-type and LEACO1_(0.821 kb)-ipt chrysanthemum plants.

FIG. 10. Bud count on LEACO1_(0.821 kb)-ipt (#5 left) was nearly 7-times higher than on wild-type plants (right) grown under similar conditions. LEACO1_(1.821 kb)-ipt (#1) and LEACO1_(0.821 kb)-ipt (#14) are shown between the wild-type and LEACO1_(0.821) kb-ipt (#5). In a following study that included additional transgenic lines, bud count on LEACO1_(0.821 kb)-ipt (#16) averaged 10-times higher than the wild-type.

FIG. 11. Flower bud number in tobacco wild-type and LEACO1_(0.821 kb)-ipt transgenic lines N2 and N4 (T₂ generation).

FIG. 12. Structure of the tomato ACO1 promoter. The position of the two repeat regions (RPT) which contains sequences with homology to the ethylene responsive promoters of 2A11 and E4 are shown. The position of the ethylene responsive (ERE) regions and stress related (TCA) motifs are also shown. The −1855 to −396 region of the promoter confers ethylene-dependent expression whereas the −396 region confers ethylene-independent expression of LEACO1_(0.821 kb)-GUS promoter fusions.

FIG. 13. LEACO1_(0.821 kb)-ipt tobacco lines displayed morphological traits that were characterized into two distinct phenomic groups. LEACO1_(0.821 kb)-ipt plants in the first group, including lines N2 and N8, displayed a relatively normal shoot morphology but with an increased number of flower buds (A) relative to the wild-type line (B). LEACO1_(0.821 kb)-ipt plants in the second group, including lines N1 and N4, displayed short internodes, increased lateral branching and poor root development (D) compared to the wild type (C).

FIG. 14A-D. Tobacco seedlings transformed with the LEACO1_(0.821 kb)-gus reporter gene. The blue color indicates increased expression of the LEACO1_(0.821 kb)-gus gene and reduced blue color indicates a reduction in gene expression. A: gus expression in young leaf, stem and root of a LEACO1_(0.821 kb)-gus transgenic seedlings (left). gus expression viewed in longitudinally sectioned shoot tips from LEACO1_(0.821 kb)-gus transgenic plants (right). Note that the strongest gus expression (indicated by arrows) is found in the apical and lateral meristems in vegetative shoots (I) and surrounding the developing flower bud and in lateral meristems in generative shoots (II); B, C & D: gus-response of transgenic LEACO1_(0.821 kb)-gus plants following exposure to IAA, ethephon, the IAA transport inhibitor TIBA, the biosynthetic precursor of ethylene ACC, or the ethylene biosynthesis inhibitor AOA in plants N5 and N3 with the shoot apex either intact (I) or removed (II). In the initial experiment, (B) IAA and TIBA applied in a lanolin paste, but AOA was applied in solution using a paintbrush to spread a thin film over the stem surface. IAA was applied to the shoot apex and TIBA was applied as a ring on the stem just below the shoot apex. In the following experiment (C & D), ACC, AOA, and ethephon were applied as sprays but TIBA was again applied in a lanolin paste.

FIG. 15. Growth characteristics and cytokinin concentrations in leaco1_(-0.821 kb)-ipt chrysanthemum lines. (top left) Vegetative branching habit of wild-type and leaco1_(-0.821 kb)-ipt chrysanthemum. The leaco1_(-0.821 kb)-ipt lines produced a highly branched, compact growth form that is most aesthetically desirable for ornamental plants. (top right) Example of the range of flowering responses for three leaco1_(-0.821 kb)-ipt chrysanthemum lines (foreground) compared to the wild-type (background). The dramatic increase in branching and flower bud number associated with the leaco1_(-0.821 kb)-ipt plants. (Bottom left) Root growth of leaco1_(-0.0821 kb)-ipt plants was unaffected by expression of the leaco1_(-0.821 kb)-ipt gene. (Bottom right) Cytokinin concentrations in the leaco1_(-0.821 kb)-ipt transgenic lines reflected the dramatic changes in phenotype observed in this study. Transgenic plants with more branching in the vegetative stage (N1 & N14) showed either a higher active cytokinin pool or evidence of increased cytokinin cycling (increase storage and deactivated pools). Line number 5 appeared similar to the wild-type in the vegetative stage but produced dramatically more buds in the reproductive mode (and a corresponding big increase all cytokinin pools.

FIG. 16. Growth habit wild-type and selected leaco1_(-0.821 kb)-ipt chrysanthemum lines. (lower right) RT-PCR analysis shows a strong correlation between the intensity of the mRNA signal and the increase in branching and flower bud number in the leaco1_(0.821 kb)-ipt plants. Note that line #3 that has a phenotype similar to the wild-type shows no mRNA transcript (does not express the ipt gene) while line #14 shows a dramatic increase in bud and branch number, a corresponding high level of gene expression (mRNA) and high cytokinin concentrations (see FIG. 15, bottom center). Bud counts for wildtype plants and selected transgenic lines grown in the growth chamber.

FIG. 17. Structures of used LEACO1_(0.821 kb)-ipt-nos construct (A) and 0.821 kb fragment of the LEACO1 promoter (B).

A: Scheme showing the structure of the LEACO1_(0.821 kb)-ipt-nos construct. From left to right: RB—right border of pBin19; P-nos nopaline synthase promoter; NPTII—neomycin phosphotransferase (nptII) gene from Tn5; T-nos—nopaline synthase terminator; LEACO1_(0.821 kb) fragment of LEACO1 promoter from tomato; U—0.97 kb 5′ UTR sequence; IPT—ipt gene from Agrobacterium tumefaciens; LB—left border of pBin19 vector. B: Scheme showing location of stress-responsive short motifs, TGTCTC (SEQ ID NO: 13)/GAGACA (SEQ ID NO: 14)-elements and G-box motifs in 0.821 kb fragment of LEACO1 promoter from Lycopersicon esculentum. Used LEACO1 promoter's fragment contained part of LTR element (between nucleotides −821 to −590 upstream from the coding start site), two 10 bp TCA motifs (↓) and an 8 bp ethylene responsive element (▮). Single copies of the consensus AuxRE TGTCTC (SEQ ID NO: 13)- and the inverse AGAACA-sequences are located at −776 and −592, respectively (

). In forward orientation the TGTCTC (SEQ ID NO: 13) element (with one substitution TGTCTt (SEQ ID NO: 15)) appears at −187, −666, and −688 (

). The G-box motif CACGTG (with one substitution CtCGTG (SEQ ID NO: 16)) appears at −552 and −656 (

). G-box core ACGT (SEQ ID NO: 17) elements were found at −483, −703 and −726(

).

FIG. 18. Poinsettia Transformation Protocol: (top left) Stem internode explants were inoculated with Agrobacterium carrying the transgene of interest. TDZ was used to induce callus, which then gave rise to shoot initials. Transgenic tissue was selected using kanamycin & transgenic shoots gradually develop from the transgenic calli (top right). Leaf from ‘Red Success’ plant transformed with 35s-gus gene (bottom). The blue colored-stain is a visual indicator of GUS activity in gus transgenic tissue.

FIG. 19 depicts SEQ ID NO:1.

FIG. 20 depicts SEQ ID NO:2.

FIG. 21 depicts SEQ ID NO:3.

FIG. 22 depicts SEQ ID NO:4.

FIG. 23 depicts SEQ ID NO:5.

FIG. 24 depicts SEQ ID NO:6.

FIG. 25 depicts SEQ ID NO:7.

FIG. 26 depicts SEQ ID NO:8.

FIG. 27 depicts SEQ ID NO:9.

FIG. 28 depicts SEQ ID NO:10.

FIG. 29 depicts SEQ ID NO:11.

FIG. 30. depicts SEQ ID NOS:12, 13-17, 11, 18-19 & 10, respectively in order of appearance.

FIG. 31 depicts SEQ ID NO:13, the sequence required for auxin responsive elements (AuxRE) in genes regulated by the auxin response factors. The sequence is shown in the forward orientation.

FIG. 32 depicts SEQ ID NO:14, the sequence required for auxin responsive elements (AuxRE) in genes regulated by the auxin response factors. The sequence is shown in the inverse orientation.

FIG. 33 depicts SEQ ID NO:15, the sequence required for auxin responsive elements (AuxRE) found in genes regulated by auxin response factors. The sequences are shown in the forward orientation with one substitution in position six (substituted bases in lower case letters).

FIG. 34 depicts SEQ ID NO:16, the sequence of the G-box motif, a regulatory element found in many genes including auxin responsive genes. The sequence is show in the forward orientation with one substitution in position two (substituted bases in lower case letters).

FIG. 35 depicts SEQ ID NO:17, the sequence of the G-box motif core elements. The sequence is shown in the forward orientation.

DETAILED DESCRIPTION OF THE INVENTION

The present invention provides nucleic acids, vectors and expression cassettes that are capable of modifying cytokinin production in a plant, thus enhancing certain desirable phenotypic characteristics such as increased bud number and/or branching without causing the negative effect on root growth associated with constitutive IPT expression. The novel constructs are designed to express the ipt gene product, isopentenyltransferase (IPT), under conditions that induce a transformed plant to express an endogenous plant cytokinin when the leaco1_(-0.821 kb) fragment of the LEACO1 gene promoter, fused to the ipt gene, is activated. This is accomplished by engineering a chimera, comprising at least one leaco gene promoter, or other ethylene responsive promoter, fused to an isopentenyltransferase (IPT)-encoding DNA. When plant cells are transformed with an expression vector harboring the chimeric gene, activation of the LEACO1 promoter causes upregulation of the IPT gene producing expression of the isopentenyltransferase enzyme and increased production of endogenous cytokinin in the affected plant tissue. In the present work a 821 bp fragment of leaco1 gene was selected which contained only a portion of the LTR-like element but two copies of the TCA motif and one of the 8 bp 5′-AA/TTTCAAA-3′ (SEQ ID NO:10) ethylene responsive element. In addition, the promoter fragment used in our study contained multiple copies of the auxin responsive element (AuxRE) required TGTCTC-sequence (SEQ ID NO: 13) (or the inverse GAGACA-sequence (SEQ ID NO: 14), or the TGTCTt sequence (SEQ ID NO: 15) with one substitution in position six [substituted bases in lower case]) found in genes regulated by auxin response factors (Ulmasov et al. 1995). The 821 bp leaco1-fragment also contains the G-box motif (CtCGTG G-Box motif (SEQ ID NO: 16) with one substitution in the two position) and multiple copies of the ACGT G-box core element (SEQ ID NO: 17) (Guilfoyle et al. 1998; Hong et al. 1995). G-box motifs are regulatory elements found in many genes including auxin responsive genes such as GmAux28 (Hong et al. 1995). A common feature of genes in the auxin/IAA family, are regions containing multiple putative AuxREs (Remington et al. 2004). The objectives were to characterize the in situ phenotypic response of transgenic chrysanthemum and tobacco lines expressing IPT under the control of an ethylene/auxin-responsive _(0.821) kb fragment of the LEACO1 promoter in the absence of an exogenous ethylene signal, and to test relative changes in LEACO1_(0.821 kb) promoter activity in response to various auxin and ethylene promoting and inhibiting agents.

Cytokinin stimulates cell division and expansion, affects lateral branch development and bud initiation, and delays whole plant senescence, post-harvest leaf deterioration, low temperature induced leaf yellowing and maintains vigor in many crop plants.

Expression of the chimeric ipt (isopentenyl transferase) gene results in the production of cytokinins. IPT is an enzyme that catalyzes the rate-limiting step in cytokinin biosynthesis. Cytokinins are phytohormones with broad effects on plant growth and development, including delayed senescence and increased branching and flower bud counts. In LEACO1_(0.821 kb)-ipt chrysanthemum, increased cytokinin concentrations were closely correlated with increased branching in vegetative plants and increased flower bud counts in flowering plants. Additionally, cytokinins interact with other plant hormones such as auxins to influence lateral branch development and flower bud number. High cytokinin concentrations can also affect ethylene biosynthetic pathway activity. When the disclosed ipt gene construct is employed in accordance with the invention, the interplay of the hormones auxin and cytokinin is fairly complex in that it is mediated through the activity of the ethylene biosynthetic pathway, in turn controlled by the promoter selected for the construct (LEACO1_(0.821 kb)).

The LEACO1 gene encodes the ACC oxidase enzyme in Lycopersicon esculentum. ACC oxidase catalyzes the conversion of 1-aminocyclopropane-1-carboxylic acid (ACC) to ethylene, the last step in the biosynthesis of this plant hormone. ACC is synthesized from S-adenosylmethionine (SAM) by the enzyme ACC synthase. Blume and Grierson (1997) reported that the ACC oxidase promoter from tomato (LEACO1) is active in response to aging, wounding, ethylene, pathogen infection and treatment with methyl jasmonate and α-amino butyric acid. The LEACO1gene is inducible in a number of organs at various stages of the plant life cycle. In addition, the ACC oxidase transcripts are reported to be spatially regulated throughout flower development (Barry, et al., 1996), and LEACO1 promoter activity detected in leaves and flowers and can be induced by external factors that stimulate ethylene pathway activity such as wounding, exogenous ethylene or pathogen infection. Khodakovskaya et al (2006) discovered that LEACO1_(0.821 kb) promoter activity increased in response to auxin and was deactivated by the auxin inhibitor TIBA.

Blume and Grierson (1997) reported that 396 bp and 1825 bp fragments in the LEACO1 promoter were sufficient to drive strong gus gene expression during both leaf and flower senescence, but that a 124 bp fragment was less effective. Based on these responses, they concluded that the essential cis-acting elements are located in the region between −396 and −124 upstream of the transcription start site. However, the 1825 bp sequence contained a repetitive element found in the tomato genome that resembles the long terminal repeats (LTRs) of copia-like retrotransposons while the 396 bp sequence did not include this element. Blume and Grierson (1997) did not test promoter response to auxin.

Further, sequences with high homology (70-75%) to the 5′ flanking sequences of the ACC oxidase genes (PHACO1, PHACO3 and PHACO4) are located within 500 bp of the transcription start site. At least two different stress-responsive short motifs were present in the 1825 bp fragment but not in the 396 bp fragment. For instance, Blume and Grierson (1997) report the 10 bp TCA motif (5′-TCATCTTCTT-3′)(SEQ ID NO:11) occurs seven times (allowing two substitutions) in the LEACO1 promoter between nucleotides −667 and −1447, and an 8 bp element (5′-AA/TTTCAAA-3′)(SEQ ID NO:10) is present in three copies between nucleotides −473 and −1662. The TCA motif is present in the 5′ upstream region of over 30 stress- and pathogen-inducible genes while the 8 bp element is reportedly necessary for ethylene-response in the carnation GST1 and the tomato E4 gene promoters.

In addition, the promoter fragment used in our study contained multiple copies of the auxin responsive element (AuxRE) required TGTCTC-(SEQ ID NO: 13) (or inverse GAGACA-(SEQ ID NO: 14)) sequence found in genes regulated by auxin response factors (Ulmasov et al. 1995) and G-box motifs, which are regulatory elements found in many genes including auxin responsive genes such as GmAux28 (Hong et al. 1995). In the LEACO1 gene promoter fragment used in our study, we identified single copies of the TGTCTC (SEQ ID NO: 13), and inverse GAGACA (SEQ ID NO: 14), sequences in reverse orientation as well as three copies of the sequence TGTCTC motif with one substitution in position six (TGTCTt (SEQ ID NO: 15)) in forward orientation (substituted bases in lower case). In addition, we identified two copies of the CACGTG G-Box motif with one substitution (CtCGTG (SEQ ID NO: 16)) and three copies of the ACGT (SEQ ID NO: 17) G-box core element. (FIG. 17).

The invention has been illustrated with LEACO1_(0.821 kb)-ipt gene; however, as one of skill in the art will appreciate, the described construct is expected to provide similar effects using related and highly homologous ipt promoters. A sequence search of the GeneBank (Blast) for homology to the LEACO1_(0.821 kb) promoter reveals homology for several genes described many years ago, although these genes were not named because the functions were unknown. The original LEACO1 gene may be included in this group and its function described at a later time.

Homology exists in some of the ethylene responsive elements contained in the promoter fragment employed in the examples described herein (LEACO1_(0.821 kb)). The RPT (two repeat) region between −1722 and −590 contains homology to the ethylene responsive promoters of the 2A11 and E4 genes. Additionally, the TCA motif is known to be present in many stress- and pathogen-responsive genes, as well as ethylene-responsive elements (ERE) found in carnation GST1 and tomato E4 gene. The fragment used in the present examples also contains a portion of a repetitive element found in the tomato genome that resembles the long terminal repeats (LTRs) of copia-like retrotransposons found in other genes. Further, sequences with high homology (70-75%) to the 5′ flanking sequences of the ACC oxidase genes (PHACO1, PHACO3 and PHACO4) are located within 500 bp of the transcription start site. In the present study, a 920 bp fragment was selected that contained only a portion of the LTR-like element but two copies of the TCA motif and one of the 8 bp 5′-AA/TTTCAAA-3′ (SEQ ID NO: 10) ethylene responsive element.

The promoter fragment used in our study contained multiple copies of the auxin responsive element (AuxRE) required TGTCTC-(SEQ ID NO: 13) (or inverse GAGACA-(SEQ ID NO: 14)) sequence found in genes regulated by auxin response factors (Ulmasov et al. 1995). TGTCTC (SEQ ID NO: 13)/GAGACA (SEQ ID NO: 14) AuxREs are found in many auxin response genes (Guilfoyle et al. 1998). Composite AuxREs may contain both the TGTCTC (SEQ ID NO: 13) element and a coupling element such as a G-box motif (Guilfoyle et al. 1998; Hong et al. 1995). G-box motifs are regulatory elements found in many genes including auxin responsive genes such as GmAux28 (Hong et al. 1995). A common feature of genes in the auxin/IAA family, are regions containing multiple putative AuxREs (Remington et al. 2004). These putative AuxREs contain motifs with at least five out of six nucleotides matching the consensus TGTCTC (SEQ ID NO: 13) sequence in forward or reverse orientation (Ulmasov et al. 1997; Ulmasov et al. 1999a; Ulmasov et al. 1999b; Remington et al. 2004). Ulmasov et al. (1997, 1999b) reported that the nucleotides TGTC (positions +1 to +4) of the TGTCTC (SEQ ID NO: 13) element are essential for binding auxin response factors, while substitutions at +5 are tolerated, and the importance of position +6 is variable.

The schematic shown in FIG. 12 (Alexander and Grierson. 2002) indicates the location of some of the key ethylene and stress response elements in the LEACO1_(0.821 kb) promoter. The schematic shown in FIG. 17 indicates the location of some of the key auxin response elements and G-Box regulatory elements in the LEACO1_(0.821 kb) promoter.

The LEACO1_(0.821 kb)-gus gene was constructed. Gus is a reporter gene that allows visualization of gene expression as a blue-colored stain. This effect was used to test the effects of various hormones, hormone inhibitors, and metabolic precursors on LEACO1_(0.821 kb) promoter activity (see FIG. 14)

Tobacco, petunia, and chrysanthemum were transformed with the LEACO1_(0.821 kb)-ipt. It is believed that similar transformations in a wide variety of other plants will alter phenotypes in a similar manner; e.g., increased number of flowering meristem (i.e., shoot tips) in poinsettia. A number of crop plants with the ipt gene under the control of other promoters have been transformed, including for example cold-inducible promoter, wound-inducible promoter, and auxin up regulated promoter. Crop species include rose and flowering tobacco (N. alata), canola, watermelon and tomato.

Differences in the number of gene copies in the genome of various transformed lines (FIG. 4) were found in tobacco. While gene number represents one possible explanation for phenotypic differences, a more likely cause is the insertion “position effect” in the genome (the location of the transgene in the chromosome and on which chromosome) that causes differences in the level of the ipt gene expression. Variations in expression level of the IPT gene) appear likely to be a major reason for the phenotypic variations observed. For example, chrysanthemum phenotype was closely correlated with ipt gene expression level, as indicated by mRNA concentration (FIG. 16) and cytokinin concentration in the tissue (Table 1).

Southern blot analysis of genomic DNA isolated from the wild type tobacco and LEACO1_(0.821 kb)-ipt transgenic tobacco lines representing two distinct phenomic groups was performed. The DIG-labeled 0.52 kb fragment of the ipt gene from LEACO1_(0.821 kb)-IPT-NOS plasmid DNA was used as a probe. One or two copies of the ipt gene were detected in lines showing either the highly branched morphology (FIG. 4C, lanes 2 and 3) or the normal shoot phenotype with increased flower bud number (FIG. 4C, lanes 4 and 5). Non-transformed wild type Nicotiana tabacum DNA (FIG. 4C, Lane 1) served as a negative control and the ipt fragment was not detected. Plasmid DNA was used as a positive control (FIG. 4C, Lane 6).

The LEACO1_(0.821 kb) promoter was used to investigate the effects of ethylene biosynthetic pathway-regulated ipt expression on the morphological development of tobacco and chrysanthemum plants grown in situ in the greenhouse and in controlled environment chambers. LEACO1_(0.821 kb)-ipt transgenic tobacco lines were sorted into two distinct groups based on overall plant growth habit and flower bud initiation (FIG. 13) while transgenic chrysanthemum lines displayed a continuous array of phenotypes from ones that appeared similar to the wild-type in branch and bud number to ones with dramatic increased in both branch and bud numbers (Table 2). In tobacco, the first phenotypic group was characterized by normal shoot morphology but showed a dramatic increase in the number of flower buds (FIG. 13A), in comparison with wild-type bud count in FIG. 13B and plant form, FIG. 13C. RT-PCR revealed low expression in the vegetative plant under glasshouse conditions. In chrysanthemum, all transgenic lines showed horticulturally acceptable shoot morphology but in some lines increases in bud counts and branch number were dramatic while in other lines the changes in bud counts and branch numbers were subtle. As in tobacco, phenotypic differences were associated with a corresponding change in gene expression, as determined by both RT-PCR (FIG. 16) and tissue cytokinin concentrations (Table 1).

In tobacco, the phenotypy of some lines were characterized by a number of dramatic changes in vegetative development but little change in generative development. The lateral shoot tips appeared abnormal and flower buds may have aborted at an early stage of development (FIG. 13D). The phenotype of these plants appeared to be typical of plants that over-express IPT. For instance, the plants in these lines tended to be short with shorter internodes. Lateral shoot development was not inhibited as is typical in tobacco, and root growth was poor. Also, ipt gene expression as determined by RT-PCR analysis, was visibly higher in lines exhibited this phenotype. In addition, transgenic plants that overproduce cytokinins typically display resistance to leaf senescence under stressful conditions. Detached leaves from LEACO1_(0.821 kb)-ipt plants displayed chlorophyll retention characteristics that correlated with the range of ipt expression levels associated with the two phenotypic groups. In contrast, transgenic chrysanthemum never displayed “abnormal’ shoot growth, even in lines with the highest expression levels; i.e., exhibiting the most lateral branching and the highest bud counts. Further, root growth appeared normal even in LEACO1_(0.821 kb)-ipt lines that displayed the more dramatic phenotypes (e.g., line N14 see FIG. 14A).

In tobacco, the increase in cytokinin concentrations in flowering LEACO1_(0.821 kb)-ipt line N5 chrysanthemum supports an increase in ipt expression when plants switch from vegetative to generative development. In the N5 chrysanthemums, plants in the vegetative stage produced cytokinin concentrations similar to the wild-type but in the generative state the active cytokinin pool increased over 3-fold, the storage cytokinin pool increased over 4-fold, and the pool of deactivated cytokinin increase 65-fold (Table 1). Under generative growth conditions, a direct increase in ethylene biosynthetic pathway activity, or a change in endogenous IAA concentration that triggered an increase in ethylene pathway activity, would be expected to result in a subsequent increase in expression of the LEACO1_(0.821 kb)-ipt gene. Previous reports indicated that IAA stimulates ethylene production by inducing expression of the ACC oxidase gene. Using the LEACO1_(0.821 kb)-gus gene to assess LEACO1_(0.821 kb)-regulated gene activity, removal of the endogenous auxin source (the shoot apex) inhibited gus gene expression. However, gus gene expression was restored by applying exogenous IAA to the excised shoot tip (FIG. 14).

In shoots with the apex intact, the auxin transport inhibitor TIBA suppressed gus expression. Shoots with the apical bud removed continued to show gus gene expression when exposed to the ethylene pathway precursor ACC but gus gene expression was suppressed in shoots with the apical bud intact when exposed to the ethylene pathway inhibitor AOA (FIG. 14B-D). Intact shoots continued to show gus gene expression when exposed to ethephon, a compound that is degraded in the plant tissue to generate ethylene.

These data indicated that the LEACO1_(0.821 kb) promoter is induced by ethylene biosynthetic pathway activity, and also demonstrated a role for endogenous auxin in triggering LEACO1_(0.821 kb) promoter activity. Blume and Grierson (1997) reported an increase in LEACO1 promoted gus expression in plants exposed directly to ethylene. In their study, gus expression was similar when promoted by either a 396 bp or a 1825 bp fragment of the LEACO1 gene promoter. While the 1825 bp fragment contained a number of short motifs that have been reported to be important for regulating many genes involved in stress response during senescence or for ethylene response the 396 bp fragment did not include any of these short motifs. In the present study, the 821 bp fragment of LEACO1 used to drive IPT (and GUS) expression included two copies of the TCA motif and one copy of the 8 bp ethylene responsive element. In addition, five copies of the required sequence for AuxREs and five copies of the G-box regulatory element or the G-box core sequence were included.

Our observation with LEACO1_(0.821 kb)-gus and LEACO1_(0.821 kb)-ipt in response to the ethylene generating compound ethephon raises an interesting questions about the interplay of various plant hormones in regulating LEACO1_(0.821 kb) activity. In LEACO1_(0.821 kb)-gus with intact apical buds, GUS expression remained high when plants were exposed to ethephon. While this observation did not suggest an increase in GUS expression (GUS expression was normally high in LEACO1_(0.821 kb)-gus with intact apical buds, FIG. 14), ethephon certainly did not reduce GUS expression. However, when LEACO1_(0.821 kb)-ipt plants were exposed to ethephon, expression of the IPT gene was suppressed (based on RT-PCR analysis, FIG. 7). One would expect ethephon to stimulate ethylene pathway activity in general, and thus increase expression in genes under the control of the LEACO1_(0.821 kb) promoter. However, Liu (1997) reported that ethephon did not affect ACC oxidase mRNA levels in sunflower hypocotyls, while in mung bean hypocotyls Kim et al. (2001) observed increased ACC oxidase transcription levels and decrease ACC synthase transcription levels in response to ethylene gas.

Simple negative feedback or autoinhibition of ethylene could explain the response observed in our study. Autoinhibition of endogenous ethylene production has been described in banana fruit tissue (Vendrell and McGlasson 1971), fruits of sycomore fig (Zeroni and Galil 1976), citrus peel discs (Riov and Yang 1982), and avocado (Zauberman and Fuchs 1973). Autoinhibition of ethylene synthesis results from the reduction in ACC availability (Riov and Yang 1982). In the case of LEACO1_(0.821 kb)-ipt plants, perhaps initial increases in cytokinin concentrations upon an ethephon treatment served to stimulate ethylene biosynthesis, but additional ethylene generation could have produced a negative feedback on ethylene biosynthesis and a subsequent down regulation of the LEACO1_(0.821 kb)-ipt gene. However, if autoinhibition of endogenous ethylene production were responsible for down regulating LEACO1_(0.821 kb) promoter activity, one might expect that GUS expression would decrease in the presence of ethephon as well.

The fact that 24 hours after ethephon treatment, plants carrying the LEACO1_(0.821 kb)-ipt showed a marked decrease in mRNA from IPT gene expression may be explained with another more likely mechanism: autoinhibition of the LEACO1_(0.821 kb)-ipt gene by increased cytokinin concentrations. Although cytokinin can induce ethylene biosynthesis in plants (Vogel et al. 1998a; Vogel et al. 1998b), it has been shown that cytokinin, an antisenescence hormone, often produces physiological effects opposite of ethylene, a senescence hormone. It is therefore possible that expression of the LEACO1_(0.821 kb)-ipt gene, which leads to an increase in cytokinin concentrations in plants, may result in an inhibition of LEACO1_(0.821 kb) gene promoter activity, that is similar to the expression of the SAG12-ipt (Gan and Amasino 1995). Kim et al. (2001) found reduced ACC oxidase activity and a progressive reduction in ethylene production in mung bean hypocotyl tissue exposed to increasing concentrations of BA, and Coenen et al. (2003) reported cytokinin inhibited auxin-induced ethylene synthesis in tomato hypocotyl segments. However, it should be noted that in intact tomato seedlings, cytokinin stimulated ethylene synthesis (Coenen and Lomax 1998), and in mungbean hypocotyls exposed to the synthetic cytokinin BA, a synergistic increase in ethylene was observed in the presence of IAA (Lau et al. 1997; Yoshii and Imaseki 1982).

The observations on the effects of regulating ipt expression with a 821 bp fragment of LEACO1 promoter on plant morphology, provide another example of the interactions between hormones. The present study illustrates some of the ways that the induction of biosynthesis of one hormone in response to another can affect plant development. The data also indicate potential uses for this specific construct in commercial plant development. For example, increases in flower bud initiation and bud development, on plants that otherwise display a phenotype characterized by low bud numbers and strong apical dominance that results in few branches, are useful in a number of commercial crop plants from asexually propagated ornamental species to sexually propagated agronomic species. With asexually propagated crop species, unlike in sexually propagated species, trait stability in the primary transformants is important while stability in the seed progeny is not.

DEFINITIONS

A “transgene” refers to genetic material that is introduced, or is capable of being introduced, into cells of a host animal. Typically, once a “transgene” is introduced into the cells of the host animal, it is maintained, either transiently or permanently, by, e.g., insertion into the host genome. In preferred embodiments of the present invention, a transgene is inserted into the host genome by homologous recombination, thereby replacing the endogenous gene with the transgene. Often, a transgene contains a coding sequence, operably linked to a promoter, that encodes a protein, e.g., a marker protein that allows the detection of the transgene in the cell. “Transgenic” refers to any cell or organism that comprises a transgene.

“Nucleic acid” refers to deoxyribonucleotides or ribonucleotides and polymers thereof in either single- or double-stranded form. The term encompasses nucleic acids containing known nucleotide analogs or modified backbone residues or linkages, which are synthetic, naturally occurring, and non-naturally occurring, which have similar binding properties as the reference nucleic acid, and which are metabolized in a manner similar to the reference nucleotides. Unless otherwise indicated, a particular nucleic acid sequence also implicitly encompasses conservatively modified variants thereof (e.g., degenerate codon substitutions) and complementary sequences, as well as the sequence explicitly indicated. The term nucleic acid is used interchangeably with gene, cDNA and nucleotide.

The terms “polypeptide,” “peptide” and “protein” are used interchangeably herein to refer to a polymer of amino acid residues. The terms apply to amino acid polymers in which one or more amino acid residue is an artificial chemical mimetic of a corresponding naturally occurring amino acid, as well as to naturally occurring amino acid polymers and non-naturally occurring amino acid polymer.

The term “amino acid” refers to naturally occurring and synthetic amino acids, as well as amino acid analogs and amino acid mimetics that function in a manner similar to the naturally occurring amino acids. As to amino acid sequences, one of skill will recognize that individual substitutions, deletions or additions to a nucleic acid, peptide, polypeptide, or protein sequence which alters, adds or deletes a single amino acid or a small percentage of amino acids in the encoded sequence is a “conservatively modified variant” where the alteration results in the substitution of an amino acid with a chemically similar amino acid. Conservative substitution tables providing functionally similar amino acids are well known in the art. Such conservatively modified variants are in addition to and do not exclude polymorphic variants, interspecies homologs, and alleles of the invention.

The term “recombinant” when used with reference, e.g., to a cell, or nucleic acid, protein, or vector, indicates that the cell, nucleic acid, protein or vector, has been modified by the introduction of a heterologous nucleic acid or protein or the alteration of a native nucleic acid or protein, or that the cell is derived from a cell so modified. Thus, for example, recombinant cells express genes that are not found within the native (non-recombinant) form of the cell or express native genes that are otherwise abnormally expressed, under expressed or not expressed at all.

The term “heterologous” when used with reference to portions of a nucleic acid indicates that the nucleic acid comprises two or more subsequences that are not found in the same relationship to each other in nature. For instance, the nucleic acid is typically recombinantly produced, having two or more sequences from unrelated genes arranged to make a new functional nucleic acid, e.g., a promoter from one source and a coding region from another source. Similarly, a heterologous protein indicates that the protein comprises two or more subsequences that are not found in the same relationship to each other in nature (e.g., a fusion protein).

A “promoter” is defined as an array of nucleic acid control sequences that direct transcription of a nucleic acid. As used herein, a promoter includes necessary nucleic acid sequences near the start site of transcription, such as, in the case of a polymerase II type promoter, a TATA element. A promoter also optionally includes distal enhancer or repressor elements, which can be located as much as several thousand base pairs from the start site of transcription. A “constitutive” promoter is a promoter that is active under most environmental and developmental conditions. An “inducible” promoter is a promoter that is active under environmental or developmental regulation. The term “operably linked” refers to a functional linkage between a nucleic acid expression control sequence (such as a promoter, or array of transcription factor binding sites) and a second nucleic acid sequence, wherein the expression control sequence directs transcription of the nucleic acid corresponding to the second sequence.

The terms “identical” or percent “identity,” in the context of two or more nucleic acids or polypeptide sequences, refer to two or more sequences or subsequences that are the same or have a specified percentage of amino acid residues or nucleotides that are the same (i.e., 60% identity, optionally 65%, 70%, 75%, 80%, 85%, 90%, or 95% identity over a specified region), when compared and aligned for maximum correspondence over a comparison window, or designated region as measured using one of the following sequence comparison algorithms or by manual alignment and visual inspection. Such sequences are then said to be “substantially identical.”

The term “transduction” refers to the introduction of foreign DNA into cells of an organism (in vivo). The term “transfection” refers to the introduction of foreign DNA into cells in culture (in vitro).

The term “vector” commonly refers to a plasmid that can be used to transfer DNA sequences. Different vectors may have properties particularly appropriate for protein expression in the recipient.

“Expression vector” results in expression of inserted DNA when propagated in a suitable host cell such as a plant cell. As used herein, “cassette” may be used to designate a structure into which DNA or a vector may be inserted.

The term “substantial” as used herein refers to being nearly the same, as when expression is substantially the same from a homologous gene. In terms of substantial identity, at least 85% identity is intended.

Use of the terms “an”, “a” and “the” and similar terms used in claiming or describing the invention are intended to be construed as including both the singular and plural, unless clearly otherwise indicated or contraindicated. The terms “including”, “having” and “containing” are to be construed as open-ended in the same manner as the terms “comprising” or “comprises” are commonly accepted as including but not limiting to the explicitly set forth subject matter. The term “comprising” and the like are construed to encompass the phrases “consisting of” and “consisting essentially of”.

The methods and processes described herein may be performed in any suitable order unless otherwise indicated or clearly rendered inoperable by a modification in order.

Limited and narrow interpretation of descriptive language intended to better illustrate the invention is not to be construed as limiting in any way nor to limit the scope of the invention contemplated by the inventors.

The invention, now described generally and in some detail, will be understood more readily by reference to the following examples, which are provided by way of reference and are in no manner intended to limit the scope of what the inventors regard as their invention.

EXAMPLES Materials and Methods

Binary vector constructions. Using standard molecular cloning procedures and the primers (forward) 5′-GGTTGAGTTGTTTCCCTCTG-3′ (SEQ ID NO:1) and (reverse) 5′-GGTAAAGTGTTTTCCTAAGTG-3′ (SEQ ID NO:2), a 0.918 kb fragment from the promoter region (including the 97 bp of 5′ UTR leader sequence plus the 821 bp of the untranscribed sequence) of the Lycopersicon esculentum LEACO1 gene (referred to herein as LEACO1_(0.821 kb)) was synthesized by PCR reaction as described below. The LEACO1_(0.821 kb) promoter fragment was cloned into the HindIII-SalI sites of the pBin19 binary vector, replacing the CaMV promoter fragment from the 35S-ipt-nos construct in this plasmid. The DNA sequence of the LEACO1_(0.821 kb) promoter fragment in the established plasmid was confirmed by DNA sequence analysis (W.M. Keck Biotechnology Laboratory, Yale University, New Haven, Conn.). The binary plasmid was transferred into Agrobacterium tumefaciens strain LBA 4404 or EHA105 by electroporation.

To construct a gene containing gus under the control of the LEACO1_(0.821 kb) fragment, the pBin19-LEACO1_(0.821 kb)-ipt vector was cut by SalI and SacI releasing the ipt gene. Similarly, the gus gene was released from the pUC19-gus-nos construct by digestion with SalI and SacI. Both DNA were dephosphorylated and then LEACO1_(0.821 kb)-nos and gus fragments were ligated together. The plasmid containing the whole LEACO1_(0.821 kb)-gus-nos fragment in pBin19 binary vector was transferred into Agrobacterium tumefaciens strain LBA 4404 by electroporation.

Transformation and production of transgenic tobacco plants. Tobacco plants were transformed using the Agrobacterium-mediated transformation method. Briefly, young tobacco leaves were surface-sterilized, cut into discs and co-cocultivated with Agrobacterium tumefaciens LBA 4404 bearing the LEACO1-ipt construct or LEACO1-gus construct. Following co-cultivation, the explants were transferred to the MS medium supplemented with 0.1 mg/l α-naphthaleneacetic acid and 1 mg/l 6-benzylaminopurine. Kanamycin at 300 mg/l was used for selection and timentin at 400 mg/l was used to suppress Agrobacterium. Explants were transferred on fresh medium at 2-3 week intervals until shoots began to emerge from the transgenic calli. Excised shoots were then transferred to MS medium containing 100 mg/l of kanamycin until roots developed. Finally, rooted plantlets were transferred to pots containing Metro 510 (Scotts, Co., Marysvill, Ohio, USA) and acclimated to the growth environment at 25° C. Individual, transgenic lines were then analyzed by PCR for foreign genes integration. Seeds from primary transformants T₀ and also from generation T₁ were germinated on MS agar medium containing 100 mg/l of kanamycin.

Plant DNA extraction and polymerase chain reaction (PCR) analysis. Total DNA was isolated from leaf tissue of greenhouse grown plants (T₀ and T₁ generations) using DNeasy Plant Mini Kits (Qiagen Inc., Valencia, Calif., USA) and 250 ng of DNA was subjected to PCR reaction. The primers used to detect the recombinant DNA were (i) forward primer 6′-GGTTGAGTTGTTTCCCTCTG-3′ (SEQ ID NO:1) and reverse primer 6′-GGTAAAGTGTTTTCCTAAGTG-3′ (SEQ ID NO:2) specific for the 0.918 kb fragment (nucleotides −1-918) of LEACO1 promoter plus UTR leader; (ii) forward primer 5′-GGTCCAACTTGCACAGGAAAG-3′ (SEQ ID NO:3) and reverse primer 6′-GGCTTGCCTACTGGAAGCTTA-3′ (SEQ ID NO:4), specific for the 0.525 kb region of the ipt gene (full size—0.723 kb); PCR amplification was performed using a thermocycler (GeneAmp PCR System 2700, Applied Biosystems, Inc., Foster City, Calif., USA). Cycling conditions for both genes were 3 min at 94° C., 30 cycles of 1 min at 94° C., 1 min at 58° C., and 1 min 30 sec at 72° C., and extension at 72° C. for 5 min. The reactions involved 200 ng of DNA template, 0.2 mM of dNTPs, 0.5 μM of each primer, REDTaq PCR Buffer and 1 unit of REDTaq DNA polymerase (Sigma, Saint Louis, Mo., USA). Finally, a 10 μl aliquot of PCR product was observed under UV after electrophoresis on a 1% agarose gel with ethidium bromide. A 1-kb DNA molecular marker (Gibco BRL, Carlsbad, Calif., USA) was used as a reference to determine DNA fragment size.

Southern hybridization. Genomic DNA was isolated from transgenic plants using a DNeasy Plant Maxi Kit (Qiagen Inc., Valencia, Calif., USA) following the manufacturer's protocol. A 10 □g per sample of total genomic DNA from putative transgenic and non-transformed control plants was digested overnight by restriction with HindIII at 37° C. Digested DNA of each line was separated through a 1% agarose gel prepared in 1×TAE and fragments were transferred from the agarose gel to a nylon membrane (Amersham, Chalfont St Giles, UK) and cross-linked to the membrane by UV treatment. The ipt gene probe (0.52 kb fragment of the 0.7 kb ipt gene) was prepared with a PCR DIG Probe Synthesis Kit (Roche Molecular Biochemicals, Indianapolis, Ind.) according to the manufacturer's instructions. DNA fixed on membranes was pre-hybridized with a pre-hybridizing solution at 68° C. for 3 hours, hybridized with probe at 68° C. overnight and washed by post-hybridization solution 4 times for 15 min. at 65° C. in a hybridization oven.

Solutions used for sample hybridization, pre- and post-hybridization, and buffers for the ensuing steps were prepared as previously reported by Mercier (1998). Membranes were washed for 5 min. in 50 ml of maleate buffer (0.1 M of maleic acid and 3.0 M of NaCl) at room temperature and then incubated for 1 hour in 50 ml of blocking solution (maleate buffer plus 0.5% blocking reagent (Roche Molecular Biochemicals, Indianapolis, Ind., USA). Next, membranes were incubated for 30 min. in 20 ml of blocking solution plus anti-dioxigenin-AP, Fab fragments (Roche Molecular Biochemicals, Indianapolis, Ind., USA) diluted to 1:10,000 and then washed 4 times for 10 min. in 50 ml of the maleate buffer.

As a final step, membranes were equilibrated for 5 min. in 50 ml of substrate buffer (100 mM of Tris-HCl; 100 mM of NaCl; 5 mM of MgCl₂) and then incubated at 37° C. for 10 min in 2 ml (sandwiched between two translucent plastic pages) of substrate buffer plus chemiluminescent substrate at a 1:100 dilution (CSPD, Roche Molecular Biochemicals, Indianapolis, Ind., USA). Membranes were exposed to autoradiographic film (Kodak X-Omart AR) for 4 hours. X-ray films were developed with an automatic film processor.

Analysis of ipt expression in leaves of tobacco. Total RNA was isolated from tobacco plants by flash freezing tissue in liquid nitrogen and then grinding in a mortar with TRI reagent (Molecular Research Center, Inc., Cincinnati, Ohio, USA). For Reverse Transcription-PCR (RT-PCR) analysis, possible DNA contamination was removed from RNA samples using a DNase treatment (DNA-free™, Ambion Inc., Austin, Tex.). The first-strand cDNA was then synthesized from 1 μg of total RNA using a RETROscript™ First Strand Synthesis Kit (Ambion Inc., Austin, Tex.) following the manufacturer's instruction. For PCR, 0.5 μL of RT-mix was used in a final volume of 25 μL. The PCR reaction for the ipt gene fragment was conducted as previously described. PCR reaction products along with RT-mix and primers to 18S RNA were used as internal standards (QuantumRNA™ 18S Internal Standards, Ambion Inc.). PCR products (10 μL) were run on a 1% agarose gel.

Plant growth conditions and morphological analysis of transgenic plants. The effect of the transgene on growth and development and number of flower buds of tobacco plants was determined as follows. Shoots from each transgenic LEACO1_(0.821 kb)-ipt tobacco plant lines #2 and #4 of T₁ generation, and from the wild-type cultivar ‘Havana’ were rooted in deep 606-cell packs (Kord Products, Bramalea, Ontario, Canada) containing a Metro 510 (Scotts Co., Marysville, Ohio, USA) peat-lite medium. After six weeks, plants from each line were harvested and the following data recorded: plant height, number of nodes, leaf area per plant, number of flower buds on main stem, number of lateral branches. These parameters were used to calculate the average internode length and the average area per leaf on the upper-most lateral shoot. These data were used to determine difference in vegetative growth habit between transgenic and wild-type plants. Plants were arranged in a randomized complete block design with 10 replicated blocks. Statistical effects were determined using a two-way analysis of variance with genetic line and cold-treatment as the main effects.

The effect of the transgene on growth and development and number of flower buds of chrysanthemum plants was determined as follows. Tip cuttings from LEACO1_(0.821 kb)-IPT chrysanthemum lines 1, 5, and 14, and the wild-type plant ‘Iridon’ were rooted in Metro 510. Rooted plants were transferred to 4″ pots and moved to plant growth chambers set at 25° C. day/20° C. night temperature and lit to 300 umol/m2/s for 16-hr per day. After the plants had acclimated to the growth chamber environment, plants in one chamber were exposed to a short-day condition (10-hr of light per day) to induce flower development, the plants in the other chamber continued to grow vegetatively under long day (16-hr per day) light conditions. Plants were arranged in a replicated block array with 6-replicates per chamber.

Plants under short days were harvested and the data recorded included number of branches on each plant, length of each branch, number of flower buds on each branch, and the number of nodes on each branch. Plants under vegetative growth conditions were harvested and the following data was recorded; number of branches on each plant, length of each branch, number of side secondary branches off each primary branch, and the number of nodes on each primary branch. This experiment was repeated with new root cuttings and plants exposed to short-day (flowering) conditions. In this experiment, 18 total replicated blocks were established using three growth chambers. Each replicated block included the LEACO1_(0.821 kb)-IPT chrysanthemum lines 1, 5, and 14, and the wild-type plant ‘Iridon’. Five plants from each line were harvested and the following data was recorded; number of branches on each plant, length of each branch, plant fresh weight, plant dry weight, total buds per plant, total leaf area per plant, and date of first open bloom. Bloom open date and bloom senescence date was recorded over time for the remaining plants in each chamber.

A larger study was initiated in early spring (around February) using cuttings from LEACO1_(0.821 kb)-IPT chrysanthemum lines 6, 10, 13, 16, 17, 19, 30, 31, 32, 33, 34, 35, 36, 37, 38, 39, 40, 41, 42, 43, 44, 45, 46, 47, 48, 49, 50, 51, 52, and the non-transgenic wild-type. Plants were grown in 608 cell packs with Metro 510. Approximately two months later, each plant was pinched to a total of five nodes, and on about two weeks later the plants were exposed to short day conditions in the greenhouse to induce flowering. Plants were harvested on after about 3.5 months later and the following parameters were recorded; numbers lateral branches per plant, length of branches, number of buds per lateral, number of nodes per branch, bud diameter at anthesis, bud diameter at the onset of senescence, and the date of bud anthesis and bud senescence. From these data the average number of buds per plant, average internode length, days from flower initiation to first anthesis, and days from anthesis to senescence were calculated.

In a follow up study, eight plants from each of 26 transgenic lines and the wild-type were grown in 5-inch pots in the greenhouse until flowering. At flowering the following data was recorded; plant fresh weight, number of lateral branches on each plant, length of each lateral branch, number of nodes on each lateral branch, total number of flower buds on each lateral branch, date of first open bloom, and bud diameter on top bud. The plant lines used in this study included LEACO1_(0.821 kb)-IPT chrysanthemum lines 1, 4, 5, 6, 10, 13, 14, 16, 17, 19, 31, 32, 33, 35, 37, 38, 40, 41, 42, 43, 45, 47, 48, 49, 50, 51, 52, and the non-transgenic wild-type. Results of this study are summarized in Table 2b.

The effects of ethylene on the ipt gene expression in two transgenic tobacco plant lines (N2 and N4) was investigated by spraying plants in the greenhouse with ethephon (500 mg/l) and then sampling tissue after 1.5 days. RNA was isolated from the tissue samples, and RT-PCR analysis was conducted as previously described.

Quantification of Chlorophyll. Specific chlorophyll concentration was calculated as follows. Leaf tissue from each sample was blotted dry, weighed, and placed in a 1.5-mL Eppendorf tube. The samples were resuspended in 80% acetone, ground with a disposable pestle, and incubated in the dark for 30 min. Total chlorophyll (Chl μg mL⁻¹) was determined according to the equation: 20.2 A₆₄₅+8.02 A₆₆₃.

Application of chemicals and histochemical analysis of GUS activity. Individual transgenic LEACO1_(0.821 kb)-gus tobacco seedlings (lines N3 and N5 of T₁ generation), that showed positive β-glucuronidase activity, were treated with either IAA, the ethylene synthesis inhibitor aminooxyacetic acid (AOA), the auxin transport inhibitor 2,3,5-triiodobenzoic acid (TIBA), the ethylene precursor 1-aminocyclopropane-1-carboxylic acid (ACC), or the ethylene generating compound ethephon. AOA, ACC, IAA, TIBA were from Sigma (Sigma-Aldrich, Inc., St. Louis, Mo., USA). Ethephon was from Rhone-Poulenc Ag Company (Monterey, Calif., USA). In the initial experiment, 100 mg/l IAA in lanolin was applied to the apex of an excised shoot, 2500 mg/l TIBA was applied in a lanolin ring directly below the intact apex, and 0.5 mM AOA was brushed on the stem surface below the apex.

In a second experiment, ACC (10⁻⁵ M), ethephon (500 mg/l) and AOA were applied as sprays but TIBA was applied as previously described. ACC was applied to seedlings that had the shoot apex removed, and the other compounds were applied to plants with the apex intact. All chemicals were reapplied every 2 days, and after six days the seedlings were harvested and histochemical analysis was conducted. In both experiments, untreated seedlings with the apex intact or with the apex removed were used as control treatments.

For histochemical assays of β-glucuronidase activity, the stems of young LEACO1_(0.821 kb)-gus tobacco seedlings were sectioned by hand. Stem sections were vacuum infiltrated with a staining solution containing 1 mM X-GLUC (5-bromo-4-chloro-3-indolyl-β-D-glucuronic acid) and incubated at 37° C. for 24 h. After staining, samples were rinsed with water and fixed in 70% ethanol. Each treatment was sampled in triplicate. Results of GUS-activity were documented using digital photography (Olympus 3× optical zoom and Olympus light microscope (SZH10) with 0.7× magnification).

The following examples are provided as illustrations of the invention and are in no way to be considered limiting.

Example 1

Transformation of tobacco. Tobacco plants were transformed using Agrobacterium-mediated transformation method. Young tobacco leaves were surface-sterilized, cut in discs and co-cocultivated with Agrobacterium tumefaciens LBA 4404 bearing the LEACO1_(0.821 kb)-ipt construct or LEACO1_(0.821 kb)-gus construct. Following co-cultivation, the explants were transferred to the MS medium (Murashige and Skoog, 1962) supplemented with 0.1 mg/l α-naphthaleneacetic acid and 1 mg/l 6-benzylaminopurine. Kanamycin at 300 mg/l was used for selection and timentin at 400 mg/l was used to suppress Agrobacterium. Explants were transferred on fresh medium at 2-3 week intervals until shoots began to emerge from the transgenic calli. Excised shoots were then transferred to MS medium containing 100 mg/l of kanamycin until roots developed. Finally, rooted plantlets were then transferred to pots containing Metro 510 (Scotts, Co., Marysville, Ohio) and acclimated to the greenhouse. Individual, transgenic lines were then analyzed by PCR (FIG. 4) to confirm integration of the foreign gene. Seeds from primary transformants T₀ and also from generation T₁ were germinated on MS agar medium containing 100 mg/l of kanamycin (FIG. 4).

Example 2

Transformation of petunia and chrysanthemum. Leaves of young (1 month old) petunia (cv. Marco Polo Odyssey) were sterilized with 10% Clorox for 15-20 min. and then rinsed 5-times with sterile water. The young, soft stems of chrysanthemum plants (cv. Iridon) were washed for 60 sec with 70% ethanol, rinsed 3-times with sterile water, and then sterilized in 5% Clorox for 8 min. before finally rinsing 5-times with sterile water. The bacterial suspension was cultured in LB medium supplemented with 50 mg/L kanamycin and 25 mg/L rifampicin. The suspension was incubated at 25° C. on a rotary shaker (220 rpm) until achieving an optical density of 0.4-0.7 (λ600 nm). The suspension was then centrifuged and the pellet re-suspended in a fresh liquid MS medium.

Leaf explants of petunia or stem segments of chrysanthemum were soaked in the infection medium for 5 min., blotted dry and kept 3 days in the dark at 22-25° C. on plates with MS medium containing 2 mg/L of N⁶-benzyladenine (BA), 0.01 mg/L of NAA for petunia explants or 0.225 mg/L of BA, 2 mg/L of IAA for chrysanthemum explants. After 2-3 days, explants were transferred to the respective selection media containing 50 mg/L of kanamycin (for selection) and 200 mg/L of timentin (to eliminate the Agrobacterium). Explants were transferred to fresh medium every 2-3 weeks, until shoots developed. Excised shoots were then transferred to phytohormone-free MS medium containing 50 mg/L of kanamycin and 100 mg/L of timentin until root induction was evident. Rooted explants were transferred to a peat-based medium, Metro 510 (Scotts Co., Marysville, Ohio) and acclimated to the greenhouse.

Example 1

Protocol for Poinsettia Transformation. Poinsettia explants were transformed using Agrobacterium-mediated transformation method. Young poinsettia stems were harvested from the greenhouse, the leaves removed and the stems surface-sterilized in 5% chlorox solution by lightly brushing the stem surface for six minutes. Stem internode sections are then cut into segments 0.3-0.5 cm long and then cut again longitudinally (FIG. 4 b). The section are plated on MS medium (with N&N vitamins and 0.1 mg/l TDZ) for a 5-day preculture period. After preculture explants are individually dipped into a broth of Agrobacterium tumefaciens LBA 4404 bearing the LEACO1_(0.821 kb)-ipt construct or LEACO1_(0.821 kb)-gus construct for 0.5 sec and then immediately blotted dry on sterile paper. The Agrobacterium inoculated explants are co-cultured for 2-4 days, and then plated onto selection medium [MS medium (Murashige and Skoog, 1962) supplemented with 0.1 mg/l TDZ and N&N vitamins] containing kanamycin and timentin at 400 mg/l. For the poinsettia cultivar ‘Red Success’ a kanamycin concentration 9-10 mg/l is used for selection. For the poinsettia cultivar ‘Winter Rose Dark Red’ a kanamycin concentration 0.5-1 mg/l is used for selection. Explants were transferred on fresh medium at 2-3 week intervals until a callus mass forms and begins to produce shoot initials. The shoots are then excised, transferred to hormone free media until root initials form. Finally, rooted plantlets were then transferred to pots containing Metro 510 (Scotts, Co., Marysville, Ohio) and acclimated to the greenhouse.

Cytokinin levels in the vegetative shoots of wild-type compared with the transformed plants are shown in Table 1. Growth characteristics of transgenic chrysanthemum plants are illustrated in FIG. 15.

TABLE 1 Cytokinin concentrations in wild-type and transgenic LEACO1_(0.821kb)-ipt chrysanthemum plants (lines, 1, 5, 14). Cytokinin types (amount in pmol g⁻¹ DW) Total Mono- Cis-form Cis-form Genetic Total Total Total phosphate pool pool line active¹ storage² deactivated³ forms⁴ (active)⁵ (storage)⁶ Vegetative shoots Wild 47.8 ± 10.1   55 ± 8.5 38.0 ± 8  75.7 ± 15.1 20.5 ± 7.8 856 ± 55 type LEACO1_(0.821kb)- 29.8 ± 5    75 ± 31 66.5 ± 38 45.7 ± 16.3 12.1 ± 2.9  920 ± 126 ipt N1 LEACO1_(0.821kb)- 75.1 ± 28.5 108 ± 28 89.2 ± 29 46.2 ± 19.9 44.5 ± 2.1 1189 ± 143 ipt N14 LEACO1_(0.821kb)-  41 ± 9.6   51 ± 0.7  44.2 ± 2.2 72.9 ± 13.9 12.3 ± 3.6 847 ± 80 ipt N5 Generative shoots LEACO1_(0.821kb)-  187 ± 40.6 167 ± 28  2979 ± 411 15.4 ± 7.1  162.1 ± 49.9   539 ± 43.8 ipt N5 Statistical effects P ≦ 0.001 P ≦ 0.01 P ≦ 0.0001 P = 0.08 P ≦ 0.01 P ≦ 0.01 Active pool: Z, DHZ, Z9R, DHZ9R, iP, iPR, iP9R Storage pool: ZOG, DHZOG, Z9ROG, DHZ9ROG Deactivated pool: Z7G, DHZ7G-1, DHZ7G-2, Z9G, DHZ9G, iP7G, iP9G Total Mono-phosphate forms ZMP, iPMP Cis-form pool (active): c-Z, c-Z9R ⁶Cis-form (Storage) c-ZOG, c-Z9ROG Z, trans-zeatin; Z9R, zeatin 9-riboside; Z9ROG, zeatin 9-riboside O-glucoside; ZMP, zeatin monophosphate; ZOG, trans-zeatin O-glucoside; Z7G, trans-zeatin-7-glucoside; Z9G, trans-zeatin-9-glucoside; DHZ, dihydrozeatin; DHZOG, dihydrozeatin O-glucoside; DHZ7G-1, dihydrozeatin-7-glucoside-1; DHZ7G-2, dihydrozeatin-7-glucoside-2; DHZ9G, dihydrozeatin-9-glucoside; DHZ9R, dihydrozeatin-9-riboside; DHZ9ROG, dihydrozeatin riboside-O-glucoside, iP, Isopenenyl adenine; iP7G, Isopenenyl adenine-7-glucoside; iP9G, Isopenenyl adenine-9-glucoside; iPR, Isopentenyl adenosine; iP7R, Isopentenyl adenosine 7-riboside; iPMP, isopentenyl monophosphate.

Table 2 shows phenotypic characteristics of chrysanthemum transformants compared with wild-type flowering performance of leaco1_(0.821 kb)-ipt chrysanthemum lines under greenhouse conditions. Plants were grown in the greenhouse in 2004 in 608 cell packs. Transgenic plants showed a wide range of branching and flowering phenotypes. Relative to control, some transgenic lines produced only 10% more flower buds but most lines (19 out or 29) showed a 50% (or greater) increase in bud count. Further, five transgenic lines produced an 8 to 10 fold increase in flower buds relative to the wild-type plant. The LEACO1_(-0.821 kb)-ipt gene similarly influenced branch development. Of the 29 transgenic lines tested in this study, 12 displayed an increase in branching habit ranging from 130% to over 340% of the number produced by the wild-type line. Correlation between level of gene expression and variation in plant form for wild-type and several LEACO1_(-0.821 kb)-ipt lines is illustrated in FIG. 16.

Table 3 shows phenotypic characteristics of chrysanthemum transformants compared with wild-type flowering performance of leaco1_(-0.821 kb)-ipt chrysanthemum lines under greenhouse conditions. Plants were grown in the greenhouse in 2005 in 5-inch pots. As in Table 2, the 27 lines tested showed a wide range of branching and flowering phenotypes

TABLE 2 Leaco1-IPT Chrysanthemum lines: Flowering performance evaluation 2004 Sort Basis: Average NO# buds per plant Average Percent (%) Average Average Average Average diameter relative total bud Average NO# lateral Average internode diameter buds buds at Days from Days from count per plant NO# buds laterals length NO# buds length at anthesis senescence initiation to anthesis to (relative to wild- Genetic line per plant per plant (cm) per lateral (mm) (mm) (mm) anthesis senescence type) Wild-type 15.5 2.67 18.7 5.8 10.5 18.7 57.0 53.7 33.3 100 leaco1-ipt 36 16.8 2.83 25.3 5.9 11.8 18.7 47.0 65.0 38.0 109 leaco1-ipt 51 19.0 2.50 17.9 7.6 10.2 18.3 45.3 57.0 42.3 123 leaco1-ipt 44 19.3 2.50 17.5 7.7 10.6 19.0 50.0 57.7 41.3 125 leaco1-ipt 50 20.8 2.17 18.9 9.6 10.8 19.7 46.3 62.3 40.7 134 leaco1-ipt 43 21.0 2.50 20.3 8.4 12.8 19.7 49.3 56.0 37.0 135 leaco1-ipt 49 21.2 2.17 18.0 9.8 10.6 20.3 44.3 57.0 38.0 137 leaco1-ipt 30 21.3 3.17 25.7 6.7 12.5 18.3 53.3 56.3 41.0 138 leaco1-ipt 46 21.8 3.50 16.1 6.2 9.5 19.7 51.0 58.3 34.3 141 leaco1-ipt 34 23.0 3.00 24.1 7.7 11.8 18.7 58.0 55.0 41.0 148 leaco1-ipt 40 24.0 3.00 23.3 8.0 11.4 14.0 54.0 55.7 38.3 155 leaco1-ipt 47 24.0 3.17 18.2 7.6 11.1 26.7 50.3 62.0 40.0 155 leaco1-ipt 52 24.0 3.83 14.0 6.3 8.4 20.0 41.0 63.7 39.0 155 leaco1-ipt 41 24.5 3.17 23.0 7.7 10.8 17.3 53.3 56.7 41.3 158 leaco1-ipt 35 24.8 3.17 25.2 7.8 11.3 18.3 52.0 56.7 38.3 160 leaco1-ipt 42 24.8 4.00 22.0 6.2 9.4 20.0 43.7 71.7 32.0 160 leaco1-ipt 33 25.0 3.33 25.6 7.5 12.3 18.3 53.3 57.0 37.7 161 leaco1-ipt 31 29.5 3.67 24.3 8.0 12.2 19.0 44.3 66.0 34.3 190 leaco1-ipt 37 29.8 3.17 24.1 9.4 11.4 15.3 44.0 59.7 43.3 192 leaco1-ipt 32 30.0 3.33 23.2 9.0 11.4 19.3 50.0 64.7 33.7 194 leaco1-ipt 38 31.3 3.50 21.8 9.0 11.1 19.0 47.0 66.7 34.0 202 leaco1-ipt 48 32.8 3.17 16.3 10.4 10.0 19.3 51.7 58.7 38.7 212 leaco1-ipt 45 54.0 4.50 14.6 12.0 8.8 22.3 27.7 73.7 36.3 348 leaco1-ipt 6 70.3 5.00 16.4 14.1 10.5 18.3 27.7 69.0 31.7 454 leaco1-ipt 19 136.3 6.17 17.5 22.1 10.5 16.5 22.5 75.0 34.0 880 leaco1-ipt 10 136.3 7.50 14.6 18.2 8.3 18.5 26.5 83.5 28.0 880 leaco1-ipt 17 142.3 5.50 16.6 25.9 9.0 16.0 25.3 74.7 35.3 918 leaco1-ipt 13 153.2 9.17 13.8 16.7 8.3 14.5 20.0 78.5 32.5 988 leaco1-ipt 16 154.7 6.83 15.2 22.6 8.6 16.0 21.0 73.0 35.0 998

TABLE 3 Phenotypic traits of wild type and leaco1_(−0.821kb)-IPT transgenic chrysanthemum (Dendranthemum X grandiflorum cv. Iridon) lines that exhibit a range of flowering and branching characteristics. Time from Internode Flower Number of start of Genotype Lateral Total flower Shoot length on buds on flower short-days (Dendranthemum X Shoot fresh shoots per buds per length top top lateral top lateral buds per until bloom grandiflorum) Line weight (g) plant (#) plant (#) lateral (cm) (cm) (#) lateral (#) (days) Means ± (se) Cultivar ‘Iridon’ WT 87.0 (4.9) 2.9 (0.1) 23.1 (1.5) 23.2 (0.5) 1.26 (0.03)  9.6 (0.9)  8.2 (0.6) 50.6 (1.3) leaco1_(−0.821kb)-IPT N1 71.8 (4.2) 5.5 (0.3) 154.6 (7.7)  20.7 (0.6) 1.02 (0.02) 46.0 (2.0) 28.3 (1.2) 62.9 (1.6) leaco1_(−0.821kb)-IPT N4 56.9 (3.9) 2.9 (0.1) 24.6 (1.6) 17.9 (0.4) 0.94 (0.02)  9.6 (0.5)  8.6 (0.5) 53.6 (1.0) leaco1_(−0.821kb)-IPT N5 67.3 (2.6) 4.1 (0.4) 88.0 (5.3) 22.7 (0.5) 1.18 (0.03) 32.9 (2.0) 21.9 (1.3) 56.9 (1.2) leaco1_(−0.821kb)-IPT N6 59.2 (4.5) 3.6 (0.3) 77.4 (7.7) 21.8 (0.9) 1.20 (0.03) 29.9 (3.7) 21.4 (1.8) 57.3 (1.1) leaco1_(−0.821kb)-IPT N10 58.6 (4.8) 5.3 (0.3) 153.1 (7.6)  18.5 (0.4) 0.99 (0.03) 46.5 (3.6) 29.5 (1.3) 65.4 (1.7) leaco1_(−0.821kb)-IPT N13 74.7 (2.5) 5.5 (0.3) 166.0 (7.0)  20.1 (0.3) 1.04 (0.03) 52.9 (2.2) 30.6 (1.4) 60.3 (0.9) leaco1_(−0.821kb)-IPT N14 62.6 (5.3) 5.8 (0.2) 148.5 (9.4)  19.6 (0.5) 1.04 (0.02) 43.3 (4.1) 26.1 (2.1) 57.8 (1.2) leaco1_(−0.821kb)-IPT N16 68.7 (5.1) 5.1 (0.2) 158.4 (10.0) 20.4 (0.7) 1.07 (0.04) 50.8 (4.1) 31.2 (2.3) 63.3 (0.9) leaco1_(−0.821kb)-IPT N17 70.7 (3.0) 6.3 (0.3) 156.4 (7.7)  19.8 (0.5) 1.06 (0.03) 46.5 (3.2) 25.2 (1.4) 59.9 (1.5) leaco1_(−0.821kb)-IPT N19 79.0 (4.6) 6.5 (0.2) 184.9 (11.1) 19.7 (0.5) 1.05 (0.04) 48.6 (2.8) 28.5 (1.4) 62.8 (1.5) leaco1_(−0.821kb)-IPT N31 104.4 (6.4)  4.1 (0.2) 38.5 (2.5) 25.3 (0.7) 1.23 (0.03) 12.4 (0.7)  9.5 (0.6) 56.5 (1.0) leaco1_(−0.821kb)-IPT N32 89.8 (5.8) 3.3 (0.2) 32.3 (2.5) 24.7 (0.4) 1.25 (0.03) 11.6 (1.2)  9.9 (0.6) 55.8 (0.6) leaco1_(−0.821kb)-IPT N33 89.6 (4.1) 3.1 (0.1) 26.0 (1.6) 26.9 (0.5) 1.21 (0.01)  9.8 (0.7)  8.4 (0.7) 52.8 (1.0) leaco1_(−0.821kb)-IPT N35 90.3 (4.3) 3.4 (0.3) 26.6 (1.8) 27.9 (0.5) 1.34 (0.02)  9.0 (0.8)  8.0 (0.5) 53.1 (0.6) leaco1_(−0.821kb)-IPT N37 106.5 (6.8)  4.1 (0.4) 37.1 (3.2) 23.8 (0.4) 1.16 (0.02) 11.3 (0.9)  9.3 (0.8) 54.0 (1.1) leaco1_(−0.821kb)-IPT N38 89.1 (6.4) 3.6 (0.3) 34.6 (2.2) 24.4 (0.6) 1.17 (0.02) 11.6 (0.8) 10.0 (1.1) 54.4 (0.5) leaco1_(−0.821kb)-IPT N40 87.8 (3.1) 3.1 (0.1) 23.3 (0.9) 26.3 (0.6) 1.27 (0.04)  8.5 (0.6)  7.5 (0.4) 50.1 (0.8) leaco1_(−0.821kb)-IPT N41 82.2 (4.4) 3.3 (0.2) 23.3 (1.4) 25.6 (0.3) 1.26 (0.02)  8.0 (0.4)  7.2 (0.4) 51.4 (0.8) leaco1_(−0.821kb)-IPT N42 68.5 (3.8) 3.6 (0.2) 29.0 (2.7) 23.2 (0.5) 1.04 (0.01)  8.5 (0.8)  8.0 (0.7) 57.4 (1.3) leaco1_(−0.821kb)-IPT N43 62.7 (3.6) 3.1 (0.1) 26.1 (1.9) 23.9 (0.7) 1.34 (0.05)  9.5 (0.8)  8.3 (0.4) 53.0 (1.3) leaco1_(−0.821kb)-IPT N45 64.1 (3.8) 2.9 (0.2) 38.4 (2.4) 21.8 (0.5) 1.05 (0.03) 16.4 (2.0) 14.1 (1.6) 56.6 (1.3) leaco1_(−0.821kb)-IPT N47 65.7 (2.8) 3.0 (0.2) 26.5 (1.4) 26.8 (0.5) 1.36 (0.02) 11.4 (0.8)  9.0 (0.7) 54.4 (0.4) leaco1_(−0.821kb)-IPT N48 65.8 (3.5) 2.8 (0.2) 30.9 (2.5) 21.6 (0.3) 1.07 (0.02) 14.9 (1.4) 11.4 (0.8) 51.4 (0.6) leaco1_(−0.821kb)-IPT N49 59.7 (3.7) 2.9 (0.1) 28.0 (2.2) 21.6 (0.3) 1.08 (0.02) 11.5 (1.1)  9.9 (0.8) 52.4 (0.9) leaco1_(−0.821kb)-IPT N50 57.1 (3.5) 2.3 (0.2) 31.0 (2.2) 21.8 (0.4) 1.08 (0.03) 16.5 (0.8) 14.0 (0.9) 55.3 (0.6) leaco1_(−0.821kb)-IPT N52 59.4 (3.5) 3.1 (0.2) 22.0 (1.7) 17.7 (0.4) 0.96 (0.02)  8.3 (0.7)  7.1 (0.4) 52.4 (0.3) Statistical Effects P-values Between lines P ≦ 0.0001 P ≦ P ≦ 0.0001 P ≦ 0.0001 P ≦ 0.0001 P ≦ P ≦ P ≦ 0.0001 0.0001 0.0001 0.0001 F-value (critical F-value = 1.55) df(between lines) = 26 12.5 29.0 150.3 34.5 20.8 79.6 70.1 17.3 Total df = 215

Example 3

Stability of tobacco transformants. The stability of the transgene in the first (T₁) and second (T₂) seed-generations of tobacco was assessed. Results are shown in Table 3 for the T₁-generation & in FIG. 11 for the T₂-generation. Basically, the phenotype observed in the primary transformant was also observed in the seed generations.

T₁ generation LEACO1_(0.821 kb)-ipt tobacco lines displayed growth habits that could be separated into one of two distinct phenotypic groups. One transgenic line from each group was selected to characterize these two basic phenotypes (Table 3). One phenotype, typified by LEACO1_(0.821 kb)-ipt lines N2 and N8, appeared similar to the wild type in overall stature and branching habit but produced a greater number of flower buds (Table 3 and FIG. 13).

The tobacco phenotype, typified by LEACO1_(0.821 kb)-ipt lines N1 and N4, displayed a more compact branching habit with fewer flower buds than either the wild type line or the transgenic lines (N2 and N8) (Table 3 and FIG. 13). Southern hybridization analysis of genomic DNA digested with HindIII confirmed the integration of the ipt gene into the genome of the T₁ transgenic lines that exhibited distinct phenotypic characteristics, while no signals was detected in the wild type plants (FIG. 4C).

The increase in flower bud initiation associated with one LEACO1_(0.821 kb)-ipt phenotype was found to be stable in successive seed generations. For example, the trend toward increased flower bud numbers in transgenic line N2 also was observed in the T₂ seed generation. In a separate experiment, the average number of flowers per plant in the wild type was 44±3.1. In comparison, transgenic tobacco plants of the T₂ generation averaged from 84.5±6.4 flowers per plant in line N2 to only 34.3±5.5 flowers per plant in line N4.

In chrysanthemum the primary means of propagation is asexual through the use of vegetative shoot tip cuttings. A wide range of flower bud increases were observed with transgenic plants producing flower bud counts ranging 109% of the wild-type to up to 998% of the wild-type. The observed increases in bud number were consistent in repeated growth chamber and greenhouse studies. Phenotypic differences were correlated with the level of ipt expression in each transgenic line (FIG. 16). The studies were conducted with plants that were asexually propagated from the primary transformant (parent plant).

RT-PCR analysis with total RNAs extracted from the leaves of wild type and transgenic lines N2 and N4 growing under normal glasshouse conditions, and the same lines treated with the ethylene-releasing compound ethephon, showed differential levels of expression (FIG. 7). The 0.52 fragment of the ipt cDNA derived from mRNA was amplified in both transgenic lines under normal greenhouse conditions but the level of expression was much higher in the line (N4) that showed the more extreme cytokinin phenotype. Gene expression was not detected in wild type plants or in transgenic lines sprayed with ethephon (500 mg/L). These data demonstrate that the range of phenotypes observed in the various LEACO1_(0.821 kb)-ipt tobacco lines corresponded with the level of ipt expression and that ipt expression could be suppressed by exogenous application of ethephon. A similar response was noted in transgenic chrysanthemum plants exposed to an ethephon spray.

Although both petunia and chrysanthemum were transformed with the LEACO1_(0.821 kb)-ipt gene, seed generation plants were not assessed. The cultivar lines used to transform in these crops were sterile, asexually propagated lines (this is typical of many ornamental plants). Seed production is possible but requires a special long period of time. With many ornamental crops, once a commercially valuable phenotype is identified, the individual line is propagated asexually.

Example 4

Establishment and molecular analysis of transgenic plants of Nicotiana tabacum harboring the LEACO1_(0.821 kb)-ipt and LEACO1_(0.821 kb)-gus fragments. The ipt gene positioned under the transcriptional control of a 0.821 kb fragment of LEACO1 promoter was introduced to wild-type tobacco plants by Agrobacterium transformation. More than 30 kanamycin-resistant, putative transformants were regenerated, transferred to pots and successfully acclimated to glasshouse conditions.

PCR analysis confirmed the integration of the foreign gene into the genome of the putative transgenic tobacco plants (FIG. 4A-B). PCR amplifications produced the expected 0.918 kb fragment of 0.821 kb LEACO1 promoter plus the 97 bp UTR leader sequence (FIG. 4A) and a 0.52 kb fragment of the ipt gene (FIG. 4B) from both the putative transgenic lines and the plasmid DNA used as a positive control. DNA was not detected in non-transgenic wild type plants. Ten kanamycin-resistant LEACO1_(0.821 kb)-gus plants were also confirmed positive for the presence of the LEACO1_(0.821 kb) promoter by PCR and stained positive in the gus histochemical assay. Over 50 transgenic lines of LEACO1_(0.821 kb)-ipt chrysanthemum were also produced and tested for flowering and reproductive growth characteristics.

Example 5

GUS expression under the control of the LEACO1_(0.821 kb) promoter. LEACO1_(0.821 kb)-gus tobacco seedlings were used to assess the effects of endogenous auxin and ethylene pathway activity on LEACO1_(0.821 kb)-controlled gene regulation. Under glasshouse conditions, gus activity was found in leaves and stems of young LEACO1_(0.821 kb)-gus (line N5) tobacco seedlings (FIG. 14A). No gus activity was observed in roots of plants from the same line.

To assess the involvement of auxin and ethylene in inducing the LEACO1_(0.821 kb) promoter, IAA, AOA, ACC, or ethephon was applied to plants with the apical buds either intact or removed (FIG. 14 B-D). Intact apical buds produce endogenous IAA but shoots with excised apical buds do not. With apical buds intact, plants showed increased gus gene expression while shoots with the apical bud removed showed reduced gus expression (FIG. 14). However, shoots with the apical bud removed showed evidence of gus gene expression when exposed to exogenously IAA applied in a lanolin paste but not when IAA was applied together with the auxin transport inhibitor TIBA.

The ethylene biosynthesis inhibitor AOA also inhibited gus gene expression. These results suggest involvement of both auxin and ethylene in stimulating LEACO1_(0.821 kb) promoter activity.

In an ensuing experiment, young LEACO1_(0.821 kb)-gus seedlings (line N3 and line N5) were treated with a spray of either AOA, ethephon, or the ethylene precursor ACC, or lanolin containing TIBA (FIG. 14. C, D). In plants with intact apical buds, gus expression was inhibited by both TIBA and AOA. But intact shoots exposed to ethephon continued to show gene expression. Seedlings with apical buds removed showed a lower level of gus gene expression compare with plants with intact apical buds but gus expression in plants with excised apical buds was stimulated by the ethylene precursor ACC.

Example 6

Leaf senescence in LEACO1_(0.821 kb)-ipt transgenic tobacco. Leaf senescence was dramatically delayed in LEACO1_(0.821 kb)-ipt transgenic plants compared to wild type tobacco plants (FIG. 8). Excised leaves from wild type tobacco and transgenic lines N2 and N4 were stored under dark conditions (25° C.) for up to 40 days. Chlorophyll content in non-transgenic wild type leaves declined to less than 5% of the initial concentration after the 10^(th) day of dark storage and disappeared completely by the 15^(th) day. Leaves of transgenic lines showed tolerance to dark storage and maintained approximately 50% of the initial chlorophyll concentrations after 20 days in the dark. Leaves from LEACO1_(0.8218b)-ipt line N4 retained approximately 25% of the initial chlorophyll concentrations for up to 40 days in the dark. Resistance to leaf senescence appeared to be positively correlated with differences in ipt gene expression.

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1. An isolated polynucleotide, or a complement thereof, comprising a nucleic acid molecule that encodes an isopentenyl transferase (IPT) operably linked to a heterologous aminocyclopropane carboxylic acid oxidase (ACO) gene promoter, wherein said nucleic acid molecule that encodes said IPT is at least 80% identical to SEQ ID NO:5 and said heterologous ACO gene promoter comprises the nucleic acid sequence set forth in SEQ ID NO:6 or
 7. 2. The isolated polynucleotide of claim 1, where said nucleic acid molecule that encodes said IPT is set forth as SEQ ID NO:
 5. 3. The isolated polynucleotide of claim 1, wherein the nucleic acid molecule hybridizes under stringent conditions to the complement of a polynucleotide set forth as SEQ ID NO:8, wherein the stringent conditions are hybridizing in 0.5 M NaHPO₄, 7% sodium dodecylsulfate (SDS), 1 nM EDTA at 65° C. and washing in 0.1×SSC/0.1% SDS at 68° C.
 4. A vector comprising the polynucleotide of claim
 1. 5. The vector of claim 4, wherein the vector is an expression vector.
 6. A host plant cell comprising the expression vector of claim
 5. 7. The host plant cell of claim 6, wherein the plant cell is a cell from a plant selected from the group consisting of tobacco, chrysanthemum, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, watermelon and bent-grass.
 8. A transgenic plant comprising a transgene which contains a nucleic acid sequence set forth as SEQ ID NO: 5 fused with a nucleic acid having the sequence of SEQ ID NO:6 or SEQ ID NO:7.
 9. A transgenic chrysanthemum plant comprising the vector of claim
 4. 10. A transgenic plant comprising the vector of claim 4, wherein the plant is selected from the group consisting of tobacco, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, watermelon and bent-grass.
 11. A progeny of the transgenic plant of claim 10, wherein the progeny comprises said vector.
 12. A seed of the transgenic plant of claim 10, wherein the seed comprises said vector.
 13. A method for increasing number of lateral branches and flower buds in a plant, comprising transforming a plant with a transgene comprising a nucleic acid encoding isopentenyltransferase (IPT) operably linked to a heterologous aminocyclopropane carboxylic acid oxidase (ACO) gene promoter, wherein expression of said transgene in the transformed plant provides increased cytokinin levels in the transformed plant compared with a non-transformed plant of the same species.
 14. The method of claim 13, wherein the plant is selected from the group consisting of tobacco, chrysanthemum, petunia, tomato, melon, pea, poinsettia, rose, canola, flowering tobacco, watermelon and bent-grass.
 15. The method of claim 13, wherein the heterologous ACO gene promoter is a promoter from a tomato ACO gene.
 16. The method of claim 13, wherein the ACO gene promoter comprises the sequence of SEQ ID NO:7.
 17. The method of claim 13, wherein the ACO gene promoter comprises the sequence of SEQ ID NO:6.
 18. The method of claim 13, wherein indoleacetic acid (IAA) production is increased in the plant.
 19. The method of claim 13, wherein ethylene production is increased in the plant.
 20. A kit comprising a LEACO1_(0.918 kb)-ipt gene chimera comprised within a vector and instructions for use.
 21. The kit of claim 20 for use in plant transformation. 